Rapid single-molecule characterisation of enzymes involved in nucleic-acid metabolism

Author:

Mueller Stefan H12ORCID,Fitschen Lucy J12ORCID,Shirbini Afnan3,Hamdan Samir M3ORCID,Spenkelink Lisanne M12,van Oijen Antoine M12

Affiliation:

1. Molecular Horizons and School of Chemistry and Molecular Bioscience, University of Wollongong , Wollongong, New South Wales 2522, Australia

2. Illawarra Health & Medical Research Institute , Wollongong, New South Wales 2522, Australia

3. Biological and Environmental Science and Engineering Division, King Abdullah University of Science and Technology (KAUST) , Thuwal 23955-6900, Kingdom of Saudi Arabia

Abstract

Abstract The activity of enzymes is traditionally characterised through bulk-phase biochemical methods that only report on population averages. Single-molecule methods are advantageous in elucidating kinetic and population heterogeneity but are often complicated, time consuming, and lack statistical power. We present a highly-generalisable and high-throughput single-molecule assay to rapidly characterise proteins involved in DNA metabolism. The assay exclusively relies on changes in total fluorescence intensity of surface-immobilised DNA templates as a result of DNA synthesis, unwinding or digestion. Combined with an automated data-analysis pipeline, our method provides enzymatic activity data of thousands of molecules in less than an hour. We demonstrate our method by characterising three fundamentally different enzyme activities: digestion by the phage λ exonuclease, synthesis by the phage Phi29 polymerase, and unwinding by the E. coli UvrD helicase. We observe the previously unknown activity of the UvrD helicase to remove neutravidin bound to 5′-, but not 3′-ends of biotinylated DNA.

Funder

Australian Research Council

National Health and Medical Research Council

Australian Government Research Training Program Scholarship

Publisher

Oxford University Press (OUP)

Subject

Genetics

Reference49 articles.

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